Exocytosis of single chromaffin granules in cell-free inside-out membrane patches (original) (raw)

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• Published: 24 March 2003

Nature Cell Biology volume 5, pages 358–362 (2003)Cite this article

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An Erratum to this article was published on 01 May 2003

Abstract

In chromaffin cells, exocytosis of single granules and properties of the fusion pore — the first connection between vesicular lumen and extracellular space1 — can be studied by cell-attached patch amperometry2,3, which couples patch-clamp capacitance measurements4,5,6,7 with simultaneous amperometric recordings of transmitter release8,9. Here we have studied exocytosis of single chromaffin granules and endocytosis of single vesicles in cell-free inside-out membrane patches by patch capacitance measurements and patch amperometry. We excised patches from chromaffin cells by using methods developed for studying properties of single ion channels10. With low calcium concentrations in the pipette and bath, the patches showed no spontaneous exocytosis, but exocytosis could be induced in some patches by applying calcium to the cytoplasmic side of the patch. Exocytosis was also stimulated by calcium entry through the patch membrane. Initial conductances of the fusion pore were undistinguishable in cell-attached and excised patch recordings, but the subsequent pore expansion was slower in excised patches. The properties of exocytotic fusion pores in chromaffin cells are very similar to those observed in mast cells and granulocytes. Excised patches provide a tool with which to study the mechanisms of fusion pore formation and endocytosis in vitro.

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References

1. Breckenridge, L.J. & Almers, W. Currents through the fusion pore that forms during exocytosis of a secretory vesicle. Nature 328, 814–817 (1987).
   Article CAS Google Scholar
2. Albillos, A. et al. The exocytotic event in chromaffin cells revealed by patch amperometry. Nature 389, 509–512 (1997).
   Article CAS Google Scholar
3. Alés, E. et al. High calcium concentrations shift the mode of exocytosis to the kiss-and-run mechanism. Nature Cell Biol. 1, 40–44 (1999).
   Article Google Scholar
4. Neher, E. & Marty, A. Discrete changes of cell membrane capacitance observed under conditions of enhanced secretion in bovine adrenal chromaffin cells. Proc. Natl Acad. Sci. USA 79, 6712–6716 (1982).
   Article CAS Google Scholar
5. Lollike, K., Borregaard, N. & Lindau, M. The exocytotic fusion pore of small granules has a conductance similar to an ion channel. J. Cell Biol. 129, 99–104 (1995).
   Article CAS Google Scholar
6. Lollike, K., Borregaard, N. & Lindau, M. Capacitance flickers and 'pseudoflickers' of small granules, measured in the cell attached configuration. Biophys. J. 75, 53–59 (1998).
   Article CAS Google Scholar
7. Debus, K. & Lindau, M. Resolution of patch capacitance recordings and of fusion pore conductances in small vesicles. Biophys. J. 78, 2983–2997 (2000).
   Article CAS Google Scholar
8. Wightman, R.M. et al. Temporally resolved catecholamine spikes correspond to single vesicle release from individual chromaffin cells. Proc. Natl Acad. Sci. USA 88, 10754–10758 (1991).
   Article CAS Google Scholar
9. Chow, R.H., Rüden, L.V. & Neher, E. Delay in vesicle fusion revealed by electrochemical monitoring of single secretory events in adrenal chromaffin cells. Nature 356, 60–63 (1992).
   Article CAS Google Scholar
10. Hamill, O.P., Marty, A., Neher, E., Sakmann, B. & Sigworth, F.J. Improved patch-clamp technique for high-resolution current recording from cells and cell-free membrane patches. Pflügers Arch. Eur. J. Physiol. 391, 85–100 (1981).
    Article CAS Google Scholar
11. Burgoyne, R.D. et al. SNAPs and SNAREs in exocytosis in chromaffin cells. Biochem. Soc. Trans. 24, 653–657 (1996).
    Article CAS Google Scholar
12. Chow, R.H., Klingauf, J., Heinemann, C., Zucker, R.S. & Neher, E. Mechanisms determining the time course of secretion in neuroendocrine cells. Neuron 16, 369–376 (1996).
    Article CAS Google Scholar
13. Pusch, M. & Neher, E. Rates of diffusional exchange between small cells and a measuring patch pipette. Pflügers Arch. Eur. J. Physiol. 411, 204–211 (1988).
    Article CAS Google Scholar
14. Fernandez, J.M., Villalon, M. & Verdugo, P. Reversible condensation of mast cell secretory products in vitro. Biophys. J. 59, 1022–1027 (1991).
    Article CAS Google Scholar
15. Klyachko, V.A. & Jackson, M.B. Capacitance steps and fusion pores of small and large-dense-core vesicles in nerve terminals. Nature 418, 89–92 (2002).
    Article CAS Google Scholar
16. Hartmann, J. & Lindau, M. A novel Ca2+-dependent step in exocytosis subsequent to vesicle fusion. FEBS Lett. 363, 217–220 (1995).
    Article CAS Google Scholar
17. Scepek, S., Coorssen, J.R. & Lindau, M. Fusion pore expansion in horse eosinophils is modulated by Ca2+ and protein kinase C via distinct mechanisms. EMBO J. 17, 4340–4345 (1998).
    Article CAS Google Scholar
18. Fernández-Chacón, R. & Alvarez de Toledo, G. Cytosolic calcium facilitates release of secretory products after exocytotic vesicle fusion. FEBS Lett. 363, 221–225 (1995).
    Article Google Scholar
19. Wang, C.T. et al. Synaptotagmin modulation of fusion pore kinetics in regulated exocytosis of dense-core vesicles. Science 294, 1111–1115 (2001).
    Article CAS Google Scholar
20. Parsons, T.D., Coorssen, J.R., Horstmann, H. & Almers, W. Docked granules, the exocytic burst, and the need for ATP hydrolysis in endocrine cells. Neuron 15, 1085–1096 (1995).
    Article CAS Google Scholar
21. Lindau, M. Time-resolved capacitance measurements: monitoring exocytosis in single cells. Quart. Rev. Biophys. 24, 75–101 (1991).
    Article CAS Google Scholar
22. Baur, J.E., Kristensen, E.W., May, L.J., Wiedemann, D.J. & Wightman, R.J. Fast-scan voltammetry of biogenic amines. Anal. Chem. 60, 1268–1272 (1988).
    Article CAS Google Scholar

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Acknowledgements

We thank L. Kwan for cell preparation and technical assistance. This work was supported by grants from the National Institutes of Health and the Nanobiotechnology Center (a Science and Technology Center programme of the NSF) to M.L., and a grant from the Ministerio de Educación y Cultura, Spain to G.A.d.T.

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Authors and Affiliations

1. School of Applied and Engineering Physics, Cornell University, Ithaca, 14853-2501, New York, USA
   Gregor Dernick & Manfred Lindau
2. Department of Physiology and Biophysics, University of Seville, Sevilla, E-41009, Spain
   Guillermo Alvarez de Toledo

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1. Gregor Dernick
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2. Guillermo Alvarez de Toledo
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3. Manfred Lindau
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Correspondence toManfred Lindau.

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Dernick, G., Alvarez de Toledo, G. & Lindau, M. Exocytosis of single chromaffin granules in cell-free inside-out membrane patches.Nat Cell Biol 5, 358–362 (2003). https://doi.org/10.1038/ncb956

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• Received: 22 March 2002
• Revised: 17 December 2002
• Accepted: 04 February 2003
• Published: 24 March 2003
• Issue Date: 01 April 2003
• DOI: https://doi.org/10.1038/ncb956

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